首页> 美国卫生研究院文献>other >No Evidence from FTIR Difference Spectroscopy that Glutamate-189 of the D1 Polypeptide Ligates a Mn Ion that Undergoes Oxidation During the S0 to S1 S1 to S2 or S2 to S3 Transitions in Photosystem II
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No Evidence from FTIR Difference Spectroscopy that Glutamate-189 of the D1 Polypeptide Ligates a Mn Ion that Undergoes Oxidation During the S0 to S1 S1 to S2 or S2 to S3 Transitions in Photosystem II

机译:FTIR差光谱法没有证据表明D1多肽的谷氨酸189连接光系统II中从S0到S1S1到S2或S2到S3过渡期间经历氧化的Mn离子。

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摘要

In the recent X-ray crystallographic structural models of photosystem II, Glu189 of the D1 polypeptide is assigned as a ligand of the oxygen-evolving Mn4 cluster. To determine if D1-Glu189 ligates a Mn ion that undergoes oxidation during one or more of the S0 → S1, S1 → S2, and S2 → S3 transitions, the FTIR difference spectra of the individual S state transitions in D1-E189Q and D1-E189R mutant PSII particles from the cyanobacterium Synechocystis sp. PCC 6803 were compared with those in wild-type PSII particles. Remarkably, the data show that neither mutation significantly alters the mid-frequency regions (1800 − 1200 cm−1) of any of the FTIR difference spectra. Importantly, neither mutation eliminates any specific symmetric or asymmetric carboxylate stretching mode that might have been assigned to D1-Glu189. The small spectral alterations that are observed are similar in amplitude to those that are observed in wild-type PSII particles that have been exchanged into FTIR analysis buffer by different methods or those that are observed in D2-H189Q mutant PSII particles (the residue D2-His189 is located > 25 Å from the Mn4 cluster and accepts a hydrogen bond from Tyr YD). The absence of significant mutation-induced spectral alterations in the D1-Glu189 mutants shows that the oxidation of the Mn4 cluster does not alter the frequencies of the carboxylate stretching modes of D1-Glu189 during the S0 → S1, S1 → S2, or S2 → S3 transitions. One explanation of these data is that D1-Glu189 ligates a Mn ion that does not increase its charge or oxidation state during any of these S state transitions. However, because the same conclusion was reached previously for D1-Asp170, and because the recent X-ray crystallographic structural models assign D1-Asp170 and D1-Glu189 as ligating different Mn ions, this explanation requires that () the extra positive charge that develops on the Mn4 cluster during the S1 → S2 transition be localized on the Mn ion that is ligated by the α-COO group of D1-Ala344 and () any increase in positive charge that develops on the Mn4 cluster during the S0 → S1 and S2 → S3 transitions be localized on the one Mn ion that is not ligated by D1-Asp170, D1-Glu189, or D1-Ala344. An alternative explanation of the FTIR data is that D1-Glu189 does not ligate the Mn4 cluster. This conclusion would be consistent with earlier spectroscopic analyses of D1-Glu189 mutants, but would require that the proximity of D1-Glu189 to manganese in the X-ray crystallographic structural models be an artifact of the radiation-induced reduction of the Mn4 cluster that occurred during the collection of the X-ray diffraction data.
机译:在最近的光系统II的X射线晶体结构模型中,D1多肽的Glu189被指定为放氧Mn4簇的配体。为了确定D1-Glu189是否连接一个在S0→S1,S1→S2和S2→S3过渡中的一个或多个过程中发生氧化的Mn离子,D1-E189Q和D1-中各个S状态的FTIR差异光谱会发生变化。蓝藻Synechocystis sp。的E189R突变体PSII颗粒。将PCC 6803与野生型PSII颗粒中的PCC进行了比较。值得注意的是,数据表明,这两个突变均不会显着改变任何FTIR差异谱的中频区域(1800-1200 cm -1 )。重要的是,这两个突变都不会消除可能已分配给D1-Glu189的任何特定的对称或不对称羧酸盐延伸模式。观察到的微小光谱变化的幅度与在通过不同方法交换到FTIR分析缓冲液中的野生型PSII颗粒中观察到的或与在D2-H189Q突变PSII颗粒中观察到的相似(残基D2- His189位于距Mn4簇> 25Å处,并接受来自Tyr YD的氢键。在D1-Glu189突变体中不存在明显的由突变引起的光谱变化,这表明在S0→S1,S1→S2或S2→期间,Mn4簇的氧化不会改变D1-Glu189的羧酸盐拉伸模式的频率。 S3过渡。这些数据的一种解释是D1-Glu189连接了一个Mn离子,该离子在任何这些S状态跃迁期间均不会增加其电荷或氧化态。但是,由于先前对D1-Asp170得出了相同的结论,并且由于最近的X射线晶体学结构模型将D1-Asp170和D1-Glu189分配为连接不同的Mn离子,因此这种解释要求()产生额外的正电荷S 1 →S 2 跃迁过程中Mn 4 团簇上的α原子位于由α-COO-组D1-Ala344和()在S 0 →S 1期间在Mn 4 簇上形成的任何正电荷增加和S 2 →S 3 跃迁位于一个不被D1-Asp170,D1-Glu189或D1-Ala344连接的Mn离子上。 FTIR数据的另一种解释是D1-Glu189不连接Mn 4 团簇。该结论与D1-Glu189突变体的早期光谱分析是一致的,但是将要求X射线晶体结构模型中D1-Glu189与锰的接近度是辐射诱导的Mn 还原的假象。 X射线衍射数据收集过程中出现的4 簇。

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